statNoiseq: Statistical testing with NOISeq
In metaseqR2: An R package for the analysis and result reporting of RNA-Seq data by combining multiple statistical algorithms
Description
Usage
Arguments
Details
Value
Author(s)
Examples
Description
This function is a wrapper over NOISeq statistical
testing. It accepts a matrix of normalized gene counts or
an S4 object specific to each normalization algorithm
supported by metaseqR2.
Usage
1
2
statNoiseq(object, sampleList, contrastList = NULL,
statArgs = NULL, geneData = NULL, logOffset = 1)
Arguments
object
a matrix or an object specific to each
normalization algorithm supported by metaseqR2, containing
normalized counts. See also Details.
sampleList
the list containing condition names
and the samples under each condition.
contrastList
vector of contrasts as defined in the
main help page of metaseqr2. See also
Details.
statArgs
a list of edgeR statistical algorithm
parameters. See the result of
getDefaults("statistics", "noiseq") for an
example and how you can modify it.
geneData
an optional annotation data frame (such
the ones produced by get.annotation which contains
the GC content for each gene and from which the gene
lengths can be inferred by chromosome coordinates.
logOffset
a number to be added to each element of
data matrix in order to avoid Infinity on log type data
transformations.
Details
Regarding object, apart from matrix (also
for NOISeq), the object can be a SeqExpressionSet
(EDASeq), CountDataSet (DESeq), DGEList
(edgeR), DESeqDataSet (DESeq2), SeqCountSet
(DSS) or ABSDataSet (ABSSeq).
Regarding contrastList it can also be a named
structured list of contrasts as returned by the internal
function metaseqR2:::makeContrastList.
Value
A named list of NOISeq q-values, whose names are the
names of the contrasts.
Author(s)
Panagiotis Moulos
Examples
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dataMatrix <- metaseqR2:::exampleCountData(1000)
sampleList <- list(A=c("A1","A2"),B=c("B1","B2","B3"))
contrast <- "A_vs_B"
lengths <- round(1000*runif(nrow(dataMatrix)))
starts <- round(1000*runif(nrow(dataMatrix)))
ends <- starts + lengths
gc=runif(nrow(dataMatrix))
biotype=rep("protein_coding",nrow(dataMatrix))
geneData <- data.frame(
chromosome=c(rep("chr1",nrow(dataMatrix)/2),
rep("chr2",nrow(dataMatrix)/2)),
start=starts,end=ends,gene_id=rownames(dataMatrix),
gc_content=gc,biotype=biotype
)
normArgs <- metaseqR2:::getDefaults("normalization","noiseq")
normDataMatrix <- normalizeNoiseq(dataMatrix,sampleList,normArgs,
geneData)
p <- statNoiseq(normDataMatrix,sampleList,contrast,
geneData=geneData)
metaseqR2 documentation built on Nov. 8, 2020, 7:34 p.m.
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Description Usage Arguments Details Value Author(s) Examples
Description
This function is a wrapper over NOISeq statistical testing. It accepts a matrix of normalized gene counts or an S4 object specific to each normalization algorithm supported by metaseqR2.
Usage
1 2 | statNoiseq(object, sampleList, contrastList = NULL,
statArgs = NULL, geneData = NULL, logOffset = 1)
|
Arguments
object |
a matrix or an object specific to each normalization algorithm supported by metaseqR2, containing normalized counts. See also Details. |
sampleList |
the list containing condition names and the samples under each condition. |
contrastList |
vector of contrasts as defined in the
main help page of |
statArgs |
a list of edgeR statistical algorithm
parameters. See the result of
|
geneData |
an optional annotation data frame (such
the ones produced by |
logOffset |
a number to be added to each element of data matrix in order to avoid Infinity on log type data transformations. |
Details
Regarding object, apart from matrix (also
for NOISeq), the object can be a SeqExpressionSet
(EDASeq), CountDataSet (DESeq), DGEList
(edgeR), DESeqDataSet (DESeq2), SeqCountSet
(DSS) or ABSDataSet (ABSSeq).
Regarding contrastList it can also be a named
structured list of contrasts as returned by the internal
function metaseqR2:::makeContrastList.
Value
A named list of NOISeq q-values, whose names are the names of the contrasts.
Author(s)
Panagiotis Moulos
Examples
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 | dataMatrix <- metaseqR2:::exampleCountData(1000)
sampleList <- list(A=c("A1","A2"),B=c("B1","B2","B3"))
contrast <- "A_vs_B"
lengths <- round(1000*runif(nrow(dataMatrix)))
starts <- round(1000*runif(nrow(dataMatrix)))
ends <- starts + lengths
gc=runif(nrow(dataMatrix))
biotype=rep("protein_coding",nrow(dataMatrix))
geneData <- data.frame(
chromosome=c(rep("chr1",nrow(dataMatrix)/2),
rep("chr2",nrow(dataMatrix)/2)),
start=starts,end=ends,gene_id=rownames(dataMatrix),
gc_content=gc,biotype=biotype
)
normArgs <- metaseqR2:::getDefaults("normalization","noiseq")
normDataMatrix <- normalizeNoiseq(dataMatrix,sampleList,normArgs,
geneData)
p <- statNoiseq(normDataMatrix,sampleList,contrast,
geneData=geneData)
|
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